蛋白质和多肽 C 端氨基酸序列研究进展

C 端序列测定长期以来是蛋白质化学领域中的一大难题,但是生物化学与分子生物学中的许多研究表明了 C 端序列的重要性.文中介绍了 C 端测定的一些最新技术,尤其侧重于化学降解法,特别是运用商品化的 N 端分析仪器分析 C 端序列,增强了仪器的通用性.文中还推荐了几种 C 端标记进而分离 C 端肽段,然后用 Edman化学法测定 C 端序列的简便方法,有一定的可行性.     

ITS序列分析与MALDI-TOF MS质谱技术在丝状真菌鉴定中的应用

丝状真菌常用的鉴定方法为形态方法和基因鉴定方法,前者限于检验人员的知识和技能,后者操作繁琐,费用略昂贵,不适合常规开展。因此,寻找丝状真菌快速鉴定方法势在必行。本文采用VITEK MALDI-TOF MS（基质辅助激光解析电离时间飞行质谱）IVD数据库（3.0版本）对临床分离的254株丝状真菌进行鉴定,并以ITS（internal transcribed spacer 内转录间隔区）序列分析为标准,验证MALDI-TOF MS质谱技术鉴定丝状真菌的准确性。结果表明MALDI-TOF MS质谱技术可以对大部分丝状真菌实现快速、准确的鉴定,其中对毛癣菌属（100%）、毛孢子菌属（100%）、毛霉菌属（100%）、曲霉菌属（96.5%）准确率很高,对犬小孢子菌（75%）、镰刀菌属（50%）、新月弯孢霉（46.2%）准确率较低,对丝状真菌鉴定的总体准确率为86.36%,与ITS测序分析符合率为83.97%。     

蛋白质及多肽的C端分析

本文采用（异）硫氰酸化学法,以乙酸酐为活化试剂,四丁铵硫氰酸为偶联试剂,溴甲基萘为烷化试剂,将蛋白质或多肽的Ｃ端依次转化并裂解为ＡＴＨ－氨基酸,在２５４ｎｍ进行检测。分析了若干种天然的、基因工程表达的蛋白质或多肽,测定了不同长度的Ｃ端序列,并确证了Ｃ端的修饰及突变情况。为蛋白质和多肽的完整性、均一性,基因工程产品及合成多肽的质控提供了重要的Ｃ端信息。目前,可在１￣２ｎｍｏｌ水平上测定了３￣５个Ｃ端     

一种SDS-PAGE与MALDI-TOF质谱联用的方法

以尿激酶原为材料,探索一种从SDS-PAGE胶上回收蛋白质做MALDI-TOF质谱的方法.所用的回收方法包括电洗脱、脱盐、除SDS等过程.电洗脱用的是高盐阻断法,脱盐用的是超滤技术,去除SDS用的是冷丙酮沉淀法.结果证明,此方法至少对一些蛋白质（如尿激酶原和牛血清白蛋白）是可行的.     

一种用于蛋白质C端序列测定的脯氨酸乙内酰硫脲(TH-Pro)新制备方法

采用Ｌ－型脯氨酸（Ｌ－Ｐｒｏ）作为原料,三甲基硅烷异硫氰酸酯（ＴＭＳ－ＩＴＣ）作为偶联试剂制备脯氨酸乙内酰硫脲（ＴＨ－Ｐｒｏ）．产物经反相ＨＰＬＣ分离纯化,并通过氨基酸组成分析,紫外光谱扫描,质谱和核磁共振等方法鉴定．反应产率高达９６％．     

电喷雾串联质谱图的叠合与多肽序列分析

利用离子阱电喷雾串联质谱仪,在选择性改变某些食品参数的条件下对模式分子Met-脑啡肽和自行固相化学合成的7肽及其修饰产物、10肽和20肽进行碎裂处理,从而获得一系列具有一定差异的串联质谱图。选择具有适当互补性的图谱进行叠合处理,得到具有连贯性“三联套”（triplet）及“二联套”（doublet）碎片离子峰的叠合串联质谱图,据此可以方便准确地角析出多肽的氨基酸序列。实验结果表明,这种方法在多肽的质谱法测定中具有一定的实用性。     

一种新的B链C端去四肽胰岛素的研制方法

报道了将单体胰岛素前体(MIP)经胰蛋白酶和羧肽酶B两步连续酶切获得B链C端去四肽胰岛素(DTI)的方法。MIP由甲醇酵母表达,最高发酵表达量达到150mg/L。发酵液中MIP通过疏水层析,分子筛初步纯化后直接进行酶切,在胰蛋白酶酶切3h后加入抑制剂paminobenzamidine处理15min,然后直接加入羧肽酶B酶切6h,再通过反相柱纯化即可得到纯品DTI,从分子筛到最后DTI,总纯化得率达到77%。按中国药典小白鼠惊厥法测定得DTI的生物活力为22IU/mg,是胰岛素的80%,在Superdex G-75分子筛上测定DTI的解离聚合曲线,证明其是单体。     

一种SDS-PAGE与MALDI-TOF质谱联用的方法

以尿激酶的为材料,探索一种从ＳＤＳ－ＰＡＧＥ胶上回收蛋白 做ＭＡＬＤＩ－ＴＯＦ质谱的方法,所用的回收方法包括电洗脱、脱盐、除ＳＤＳ等过程,电洗脱用的是高盐阻断法,脱盐用的超滤技术,去除ＳＤＳ用的是冷丙沉淀法,结果证明,此方法至少对一些蛋白质是可行的。     

序列搜索算法在多肽质谱解析中的应用

序列搜索算法由三部分组成：搜索过程、搜索得到多肽的各氨基酸残基的评分及两端（N端、C端）搜索得到的多肽的合并过程.通过若干实际多肽质谱的解析,结果表明,该算法对多种序列专一性离子并存的未知多肽质谱的解析,可获得较满意结果.尤其是它的评分方式及标准,比较适合多肽质谱图的实际情况,可最大限度地判断解析结果的准确度,为从事用质谱测定多肽一级结构的分析工作者提供了一比较简便且可靠的手段.也为质谱法快速测定蛋白质或多肽序列及其在生物学中的普及提供了一条方便之路.     

MALDI-TOF质谱在细菌检测及鉴定中的研究进展

近年来,随着质谱技术的快速发展,软电离方式的出现,基质辅助激光解吸电离飞行时间质谱能够对蛋白质、核酸及脂类等生物大分子进行快速、准确的分析,进而使得其被应用于细菌的检测及鉴定成为可能。本文综述了当前基质辅助激光解吸电离飞行时间质谱在细菌检测及鉴定方面的研究进展。     

双向凝胶电泳银染蛋白质点的肽质谱指纹图分析

对双向凝胶电泳后银染显色的蛋白质点经脱色与原位还原和烷基化处理后,用ＴＰＣＫ胰蛋白酶进行酶解,采用带有Ｃ１８反相载体的ＺｉｐＴｉｐ＾ＴＭ吸头进行脱盐处理,再进行ＭＡＬＤＩ－ＴＯＦ肽质谱指纹纹图分析,然后将肽质数据在ＥＭＢＬ数据库中进行搜寻从而对蛋白南点进行鉴定。结果表明用该实验程序可对银染的单一蛋白南点进行快速肽质谱指纹图ｉｐＴｉｐ＾ＴＭ的应用可以明显增加质谱分析的信噪比,提高分析灵敏度。用以上方     

MALDI-TOF-MS对寡核苷酸的序列分析

通过对几种基质测定含不同碱基的寡核苷酸的灵敏度及精确度的比较,发现用混合基质α－氰基４－羟基肉桂酸（α－Ｃｙａｎｏ）／３－羟基吡啶羧酸（３ＨＰＡ）用于基质辅助激光解吸附电离飞行时间质谱中测定脱氧寡核苷酸,不仅能得到较好的分子离子峰,而且一些金属离子的加合物峰能得到有效的抑制,提高了测定的灵敏度。用３′－和５′－外切酶对脱氧寡核苷酸１２－ｍｅｒ（５′－ＡＴＧＣＡＴＡＴＧＣＡＴ－３′）进行部分降解,再进行ＭＡＬＤＩ－ＴＯＦ－ＭＳ分析,得到了完整的寡核苷酸的序列。     

Identification of Protein Markers Specific for Papillary Renal Cell Carcinoma Using Imaging Mass Spectrometry

Since the emergence of proteomics methods, many proteins specific for renal cell carcinoma (RCC) have been identified. Despite their usefulness for the specific diagnosis of RCC, such proteins do not provide spatial information on the diseased tissue. Therefore, the identification of cancer-specific proteins that include information on their specific location is needed. Recently, matrix-assisted laser desorption ionization (MALDI) mass spectrometry (MS) based imaging mass spectrometry (IMS) has emerged as a new tool for the analysis of spatial distribution as well as identification of either proteins or small molecules in tissues. In this report, surgical tissue sections of papillary RCC were analyzed using MALDI-IMS. Statistical analysis revealed several discriminative cancer-specific m/z-species between normal and diseased tissues. Among these m/z-species, two particular proteins, S100A11 and ferritin light chain, which are specific for papillary RCC cancer regions, were successfully identified using LC-MS/MS following protein extraction from independent RCC samples. The expressions of S100A11 and ferritin light chain were further validated by immunohistochemistry of human tissues and tissue microarrays (TMAs) of RCC. In conclusion, MALDI-IMS followed by LC-MS/MS analysis in human tissue identified that S100A11 and ferritin light chain are differentially expressed proteins in papillary RCC cancer regions.     

Peptide Sequencing by Mass Spectrometry for Homology Searches and Cloning of Genes

It is now possible to obtain sequence information from gel-separated proteins by mass spectrometry at levels too low for conventional approaches. Usually this tandem mass spectrometric data are used for database searches with the aim of identifying the corresponding gene. Recently it has been shown that long and accurate amino acid sequences can be obtained which are sufficient for PCR-based strategies to clone the corresponding gene [Wilm et al. (1996), Nature 379, 466–469]. More than eight proteins have now been cloned based on that method. In many more cases the sequence information identified homologous proteins. Issues involved in cloning by mass spectrometric sequence information are discussed, as are two case studies. These results clearly establish mass spectrometry as a viable tool not only for the database identification of proteins, but also for the de novo sequencing of gel-separated proteins at the low-picomole to femtomole level.     

MALDI-TOF质谱技术研究多肽一级结构特性

海兔酸性多肽(Aplysiaacidicpeptide,AAP)和海兔胰岛素Cβ(AplysiaInsulinCβ,AICβ)的一级结构分别由27和15个氨基酸残基组成,其中前者含有6个亮氨酸残基(L),并组成3对LL键,后者仅有2个亮氨酸残基,组成1对LL键。选用基质辅助激光解吸离子化飞行时间(matrixassistedlaserdesorptionionizationtimeoffight,MALDITOF)质谱技术研究AAP,AICβ和它们分解产物的一级结构稳定性过程中,发现在弱酸性介质条件下,AAP和AICβ的LL酰氨键键能比LR键能(R表示除了L以外的氨基酸残基)更强,不易被分解。AICβ和猪血管紧张肽I(angiotensinI,AnI)样品中均含有单电荷的多聚肽。随着多肽聚合数递增,多肽质谱峰的相对强度剧减。AICβ在形成多聚肽过程中,发生释放H+的现象 。     

固相化学辅助MALDI-TOF质谱源后衰变技术对2D-胶银染蛋白质点的鉴定

利用O 甲基异脲氢硫酸 (O methylisoureahydrogensulfate)修饰 2D 胶上胰蛋白酶原位酶切后产生的Lys 肽 ,使其具有Arg 肽的特性 ,提高质谱测定的灵敏度 ,然后用化学试剂 3 磺酸丙酸N 羟基琥珀酰胺酯 ( 3 sulfopropionicacidNHS ester)修饰Lys 肽及Arg 肽 ,修饰的产物在进行PSD测序时能得到单一的y 离子系列 ,有利于蛋白质酶解片段序列的从头解析 ,为 2D 胶上蛋白质点的准确鉴定提供有力的依据 ;该方法应用于鼻咽癌细胞 2D胶银染蛋白质点的鉴定取得可靠结果     

Labeling elastase digests with TMT: informational gain by identification of poorly detectable peptides with MALDI-TOF/TOF mass spectrometry

The applicability of the less specific protease elastase for the identification of membrane and cytosolic proteins has already been demonstrated. MALDI as ionization technique particularly favors the detection of basic and to a lesser extent of weakly acidic peptides, whereas neutral peptides often remain undetected. Moreover, peptides below 700 Da are routinely excluded. In the following study, the advantage of additional information gained from tandem mass tag zero labeled peptides and the resultant increase in sequence coverage was evaluated. Through derivatization with tandem mass tag reagents, peptide measurement within the standard mass range of the MALDI reflector mode is achievable due to the mass increase. Compared to the unlabeled sample, peptides exhibiting relatively low molecular masses, pI values or higher hydrophobicity could be identified.     

Analysis of chronic lung transplant rejection by MALDI-TOF profiles of bronchoalveolar lavage fluid

While lung transplant is an effective therapy for advanced lung disease, chronic allograph rejection remains a primary basis for lower survival rates than those for other solid organ transplants. This study used carefully controlled Zip-Tip extraction of bronchoalveolar lavage fluid (BALF) followed by MALDI-TOF MS to identify biomarkers of chronic lung transplant rejection. Many differences were observed between controls, those who did not develop chronic rejection within 100 months, and patients who had developed chronic rejection, diagnosed as bronchiolitis obliterans syndrome (BOS). Intensity ratios of peaks within the same MALDI-TOF profile were used to quantify the result. One of the best identifiers of BOS was a lowered ratio of clara cell protein (CCP m/z = 15,835) to lysozyme (m/z = 14,700), which gave 94% specificity and 74% sensitivity for diagnosis. Furthermore, low values for CCP/Lysozyme (<0.3) were observed in 66% of samples taken at 1 to 15 months prior to the diagnosis of BOS. Many other components of the profile gave similar or better outcomes for diagnosis but tended to be less valuable for the prediction of future disease. Overall, this study demonstrated the feasibility of this approach for the detection of disease biomarkers.     

Distinctive characteristics of MALDI-Q/TOF and TOF/TOF tandem mass spectrometry for sequencing of permethylated complex type N-glycans

Concerted MALDI-MS profiling and CID MS/MS sequencing of permethylated glycans is one of the most effective approaches for high throughput glycomics applications. In essence, the identification of larger complex type N-glycans necessitates an unambiguous definition of any modification on the trimannosyl core and the complement of non-reducing terminal sequences which constitute the respective antennary structures. Permethylation not only affords analyses of both neutral and sialylated glycans at comparable ease and sensitivity but also yields more sequence-informative fragmentation pattern. Facile glycosidic cleavages directed mostly at N-acetylglucosamine under low energy CID, as implemented on a quadrupole/time-of-flight (Q/TOF) instrument, often afford multiple losses of the attached antenna resulting in characteristic ions related to the number of antennary branches on the trimannosyl core. Non-reducing terminal epitopes can be easily deduced but information on the linkage specific substituent on the terminal units is often missing. The high energy CID MS/MS afforded by TOF/TOF instrument can fill in the gap by giving an array of additional cross-ring and satellite ions. Glycosidic cleavages occurring specifically in concert with loss of 2-linked or 3-linked substituents provide an effective way to identify the branch-specific antennary extension. These characteristics are shown here to be effective in deriving the sequences of additionally galactosylated, sialylated and fucosylated terminal N-acetyllactosamine units and their antennary location. Together, a highly reproducible fragmentation pattern can be formulated to simplify spectral assignment. This work also provides first real examples of sequencing multiply sialylated complex type N-glycans by high energy CID on a TOF/TOF instrument. Shin-Yi Yu and Sz-Wei Wu contributed equally to this work. Dedicated to the late Prof. Yasuo Inoue, without whom the body of work represented by this article would not have been initiated in Taiwan.     

Protein prenylation in an insect cell-free protein synthesis system and identification of products by mass spectrometry

To evaluate the ability of an insect cell-free protein synthesis system to carry out proper protein prenylation, several CAIX (X indicates any C-terminal amino acid) sequences were introduced into the C-terminus of truncated human gelsolin (tGelsolin). Tryptic digests of these mutant proteins were analyzed by MALDI-TOF MS and MALDI-quadrupole-IT-TOF MS. The results indicated that the insect cell-free protein synthesis system possesses both farnesyltransferase (FTase) and geranylgeranyltransferase (GGTase) I, as is the case of the rabbit reticulocyte lysate system. The C-terminal amino acid sequence requirements for protein prenylation in this system showed high similarity to those observed in rat prenyltransferases. In the case of rhoC, which is a natural geranylgeranylated protein, it was found that it could serve as a substrate for both prenyltransferases in the presence of either farnesyl or geranylgeranyl pyrophosphate, whereas geranylgeranylation was only observed when both prenyl pyrophosphates were added to the in vitro translation reaction mixture. Thus, a combination of the cell-free protein synthesis system with MS is an effective strategy to analyze protein prenylation.